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使用硫黄素T通过流式细胞术纯化阿尔茨海默病淀粉样斑块核心蛋白。

Flow cytometric purification of Alzheimer's disease amyloid plaque core protein using thioflavin T.

作者信息

Palutke M, KuKuruga D, Wolfe D, Roher A

机构信息

Department of Pathology, Wayne State University School of Medicine, Detroit, Michigan 48201.

出版信息

Cytometry. 1987 Sep;8(5):494-9. doi: 10.1002/cyto.990080510.

Abstract

Amyloid plaque core protein (APCP) of Alzheimer's disease obtained from brain tissue homogenate is difficult to recover in pure form, primarily because of contaminating lipofuscin (LF) granules. Thioflavin T, a fluorescent dye previously used to stain amyloid, was found to bind to APCP but not to lipofuscin. The latter, however, is autofluorescent. Fluorometric studies showed that at 370 nm excitation APCP has a maximal emission at 418 nm, whereas the autofluorescent LP has a maximal emission at 450 nm. This difference in emission permitted the use of a flow cytometer-sorter (FACS 440) for purification of APCP. APCP particles fluoresced distinctly from LF granules on the log blue fluorescence parameter. The two entities were sorted using forward light scatter versus fluorescence. A collection apparatus was designed and prepared to facilitate the collection of large volumes of sheath fluid and particles and to minimize fragmentation of particles during the collection process. The sorted APCP fraction was 98% pure. This work demonstrates how old dyes can be used to perform new tricks and provide a useful method for separating complex protein.

摘要

从脑组织匀浆中获取的阿尔茨海默病淀粉样斑块核心蛋白(APCP)难以以纯形式回收,主要是因为受到脂褐素(LF)颗粒的污染。硫黄素T是一种先前用于染色淀粉样蛋白的荧光染料,发现它能与APCP结合,但不与脂褐素结合。然而,后者具有自发荧光。荧光测定研究表明,在370nm激发下,APCP在418nm处有最大发射峰,而自发荧光的LP在450nm处有最大发射峰。这种发射差异使得可以使用流式细胞仪分选仪(FACS 440)来纯化APCP。在对数蓝色荧光参数上,APCP颗粒与LF颗粒发出明显不同的荧光。利用前向光散射与荧光对这两种物质进行分选。设计并准备了一个收集装置,以方便收集大量的鞘液和颗粒,并在收集过程中尽量减少颗粒的破碎。分选得到的APCP部分纯度为98%。这项工作展示了旧染料如何能用于新用途,并为分离复杂蛋白质提供了一种有用的方法。

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